Title Injectable, self-gelling, biodegradable, and immunomodulatoryDNA hydrogel for antigen delivery.
Author(s)
Nishikawa, Makiya; Ogawa, Kohei; Umeki, Yuka; Mohri,Kohta; Kawasaki, Yohji; Watanabe, Hiroshi; Takahashi,Natsuki; Kusuki, Eri; Takahashi, Rei; Takahashi, Yuki;Takakura, Yoshinobu
Citation Journal of controlled release : official journal of the ControlledRelease Society (2014), 180: 25-32
Issue Date 2014-04-28
URL http://hdl.handle.net/2433/185154
Right © 2014 Elsevier B.V.
Type Journal Article
Textversion author
Kyoto University
1
Injectable, Self-Gelling, Biodegradable, and Immunomodulatory DNA
Hydrogel for Antigen Delivery
Makiya Nishikawa,1,*
Kohei Ogawa,1 Yuka Umeki,
1 Kohta Mohri,
1 Yohji Kawasaki,
2 Hiroshi
Watanabe,2 Natsuki Takahashi,
1 Eri Kusuki,
1 Rei Takahashi,
3 Yuki Takahashi,
1 and Yoshinobu
Takakura1
1Department of Biopharmaceutics and Drug Metabolism, Graduate School of Pharmaceutical
Sciences, Kyoto University, Sakyo-ku, Kyoto 606-8501, Japan. 2Institute for Chemical Research,
Kyoto University, Gokasho, Uji, Kyoto 611-0011, Japan. 3Department of Pharmacotherapeutics,
Faculty of Pharmaceutical Sciences, Doshisha Women's College of Liberal Arts, Kyotanabe,
Kyoto 610-0395, Japan.
Corresponding Author
Makiya Nishikawa, Ph.D., Department of Biopharmaceutics and Drug Metabolism, Graduate
School of Pharmaceutical Sciences, Kyoto University, Sakyo-ku, Kyoto 606-8501, Japan.
Telephone: +81-75-753-4580. E-mail: [email protected]
ABSTRACT
DNA nanotechnology-based nanosystems and macrosystems have attracted much attention in the
biomedical research field. The nature of DNA endows these systems with biodegradable,
biocompatible, and immunomodulatory properties. Here, we present an injectable hydrogel
system that consists only of chemically synthesized short DNA strands, water, and salts. Several
preparations of polypod-like structured DNA, or polypodna, were designed, including tri-, tetra-,
penta- and hexapodna, as the building blocks of self-gelling DNA hydrogel. Under physiological
conditions, properly designed polypodna preparations formed a hydrogel. The analysis of the
modulus data of the hydrogel consisting of two sets of hexapodna preparations showed that this
injectable hydrogel was reorganized in a time scale of 0.25 s. Then, DNA hydrogel containing
unmethylated cytosine-phosphate-guanine (CpG) dinucleotides was used to stimulate innate
immunity through Toll-like receptor 9, the receptor for CpG DNA. Gel formation significantly
increased the activity of immunostimulatory CpG DNA, retarded the clearance after intradermal
injection into mice, and increased the immune responses to ovalbumin (OVA) incorporated into
the hydrogel as a model antigen. OVA/CpG DNA hydrogel induced much less local or systemic
adverse reactions than OVA injected with complete Freund’s adjuvant or alum. GpC DNA
hydrogel containing no CpG sequences was less effective, indicating the importance of
immunomodulation by CpG DNA hydrogel. Thus, we have created an efficient system for
sustained delivery of antigens or other bioactive compounds.
Keywords: hydrogel, CpG motif, controlled release, antigen, immune cell, self-gelling
2
INTRODUCTION
Natural, biocompatible, and biodegradable materials are optimal properties of potential drug
delivery systems. DNA fits these criteria because it has been naturally selected for the storage,
transmission, and expression of genetic information. Recent progress in DNA nanotechnology
research has facilitated the design and construction of a variety of DNA-based nano-sized
structures [1-5]. Although these designs are esthetically satisfying, most of these systems have
not yet been applied to the pharmaceutical or therapeutic fields.
DNA also has immunomodulatory properties when present in the cytosol or outside cells.
DNA containing unmethylated cytosine-phosphate-guanine (CpG) dinucleotides, or CpG DNA
[6,7] is a potent stimulator of innate immunity, as it is the ligand for the Toll-like receptor 9
(TLR9) [8]. CpG DNA induces the production of helper T-cell type 1 cytokines, and its clinical
potential is being investigated in several indications, including cancer [9-11]. Phosphorothioate
(PS)-stabilized CpG DNA is the form most frequently used in clinical trials [12,13], although it
is associated with renal toxicity. We propose that polypod-like structured DNA, or polypodna for
short, consisting of three or more oligodeoxynucleotides (ODNs) is a novel and alternative
approach to increasing the immunostimulatory activity of CpG DNA, without the requirement
for PS stabilization [14,15].
Connecting multiple tetrapodna (X-DNA) units results in the formation of DNA hydrogel,
as first reported by Um et al [16]. We extended these results by replacing the DNA sequences
with those containing immunostimulatory CpG motifs [17]. In these studies, palindromic four
nucleotides at the 5’-ends of ODNs were ligated using T4 DNA ligase to obtain DNA hydrogels.
The CpG DNA hydrogel containing doxorubicin was effective in inhibiting tumor growth in
mice, but the administration of the hydrogels required surgical incision, or breaking them down
into fragments small enough for injection. A more important issue with pre-existing DNA
hydrogel formulations is that the contaminating ligase can trigger unwanted responses, including
anaphylactic shock. Therefore, the development of ligation-free and injectable DNA hydrogels
would greatly improve the potency of DNA hydrogels as sustained delivery systems. There are
few reports on the preparation of DNA hydrogels without the use of DNA ligase [18,19] and no
injectable DNA hydrogels have been reported thus far.
Here we present a novel method to develop ligase-free, injectable DNA hydrogel. To this
end, the single stranded 5’-ends of polypodna were extended to hybridize under physiological
conditions. These hydrogels were easily injected using a fine gauge needle, and gelation occurs
almost instantly following injection. Finally, we show that the DNA hydrogel can efficiently
deliver tumor antigens with higher potency and less toxicity than clinically available vaccine
adjuvants.
MATERIALS AND METHODS
Animals and cell culture. Four-week-old ICR mice and six-week-old C57BL/6 mice were
purchased from Japan SLC, Inc. (Shizuoka, Japan). All animal experiments were conducted in
accordance with the principles and procedures outlined in the National Institutes of Health Guide
for the Care and Use of Laboratory Animals. The protocols for animal experiments were
approved by the Animal Experimentation Committee of Graduate School of Pharmaceutical
Sciences, Kyoto University. Mouse dendritic DC2.4 cells were a gift from Dr. K. L. Rock,
University of Massachusetts Medical School, Worcester, MA, USA. CD8OVA1.3 cells, a mouse
T cell hybridoma against an OVA class I epitope, were a gift from Dr. C. V. Harding, Case
3
Western Reserve University, Cleveland, OH, USA. EL4, a T lymphoma, and EG7-OVA, an
OVA transfectant of EL4, were purchased from American Type Culture Collection (Manassas,
VA, USA). Cell culture was performed as previously described [20].
Preparation of polypodna and DNA hydrogel. All phosphodiester ODNs were purchased from
Integrated DNA Technologies, Inc. (Coralville, IA, USA). The sequences of the ODNs are
summarized in Table S1. Polypodna preparations were prepared by mixing equimolar ODNs as
previously described [15], and the formation was confirmed by 6% polyacrylamide gel
electrophoresis (PAGE). DNA hydrogel was obtained by increasing the salt or DNA
concentration of polypodna solution, or by mixing different units of polypodna or other forms of
DNA assemblies, such as double stranded DNA (dsDNA). The hydrogel formation was briefly
checked by adding solution containing blue dextran (Sigma-Aldrich, St. Louis, MO, USA),
because it does not instantly diffuse into hydrogel. The inner structure of DNA hydrogel was
observed using a field-emission scanning electron microscope (FE-SEM: S4700, HITACHI,
Japan) as previously described [17]. The melting temperature (Tm) was obtained with a
Shimadzu UV-1600 PC spectrometer (Kyoto, Japan) equipped with a TMSPC-8 temperature
controller as previously described [15].
Measurement of viscoelastic properties of DNA hydrogel. Rheological behavior of DNA
hydrogels was examined with a laboratory rheometer (ARES; Rheometric Scientific currently
TA Instruments, USA) at room temperature (~25 C). A parallel-plate fixture with the diameter
of 8.0 mm was used for oscillatory and steady flow tests, following a standard protocol of
rheological test [21].
IL-6 release from DC2.4 cells or in mice. DNA samples were added to DC2.4 cells at the
indicated concentrations and the cells were incubated for 16 h. Then, the supernatant was
collected and the concentration of IL-6 was determined by ELISA following the manufacturer’s
protocol (BD Biosciences, San Diego, CA, USA). Serum samples of mice receiving an
intradermal injection of 220 g DNA were also subjected to ELISA.
Radiolabeling of ODN. An ODN (ssDNA(GpC)8np-32-A1) was end-labeled with 32
P using [-32
P]ATP and T4 polynucleotide kinase (T4 PNK; Takara Bio, Otsu, Japan) according to the
manufacturer’s instructions, and purified using NAP5 columns (GE Healthcare, Tokyo, Japan). 32
P-DNA was used to obtain 32
P-ssDNA(CpG), 32
P-hexapdna(CpG) or 32
P-DNA hydrogel(CpG).
Tissue distribution of radioactivity after intradermal injection of 32
P-DNA. ICR mice were
intradermally injected with 32
P-DNA at a dose of 10 mg DNA/kg (220 g DNA/mouse). At the
indicated times after injection, mice were anesthetized and the injection site and draining lymph
nodes were collected and processed as previously reported [22]. Then, the radioactivity in these
tissue samples was counted in a Tri-Carb 3110 TR counter (Perkin–Elmer, Norwalk, CT, USA).
Quantitative measurement of IL-6 mRNA expression. Under anesthesia with isoflurane,
C57BL/6 mice were injected with 220 g DNA. At the indicated time points after injection, mice
were anesthetized and the injection site and draining lymph nodes were excised. The total RNA
was extracted from the skin tissues using an RNeasy mini kit (QIAGEN GmbH, Hilden,
Germany) in accordance with the manufacturer’s protocol. Total RNA from the draining lymph
4
nodes was extracted using Sepasol RNA I super (Nacalai Tesque). The extracted RNA was
reverse-transcribed with a ReverTra Ace®
qPCR RT Kit (TOYOBO, Osaka, Japan). For
quantitative analysis of mRNA expression, real-time PCR was conducted with total RNA using
KAPA SYBR FAST ABI Prism 2X qPCR Master Mix (KAPA BIOSYSTEMS, Boston, MA,
USA). The ODN primers used for amplification were as follows: IL-6, forward (5’-
GTTCTCTGGGAAATCGTGGA-3’) and reverse (5’-TGTACTCCAGGTAGCTATGG-3’); -
actin, forward (5’-CATCCGTAAAGACCTCTA- TGC-3’) and reverse (5’-
ATGGAGCCACCGATCCACA-3’). Amplified products were detected online via intercalation
of SYBR Green, a fluorescent dye, by using StepOnePlus Real Time PCR System (Applied
Biosystems, Foster City, CA, USA). The IL-6 mRNA expression was normalized to the mRNA
level of -actin.
OVA release from DNA hydrogel. OVA (albumin from chicken egg white, Sigma-Aldrich)
was labeled with fluorescein isothiocyanate (FITC; fluorescein isothiocyanate isomer 1, Sigma-
Aldrich) to obtain FITC-OVA. FITC-OVA was added to both hexapodna solutions and DNA
hydrogel was prepared by mixing the solutions. Then, FITC-OVA/DNA hydrogel (10 l) was
placed into the upper chamber of the Transwell (Product#3460, 0.4 m pore size, Corning Inc.,
Corning, NY, USA), and 500 l PBS was added into the bottom chamber, and incubated at 37 C.
At predetermined time points, bright field and fluorescence images of FITC-OVA/DNA
hydrogel were obtained using LAS3000 system (Fujifilm, Tokyo, Japan), and the receiver
solution was collected and replaced with 500 l fresh PBS. The fluorescence intensity of the
receiver solution was measured in a Wallac 1420 ARVO MX-2 Multilabel Counter (Perkin
Elmer, Boston, MA, USA).
Degradation of DNA hydrogel by DNase. Hexapodna preparations (220 μg/100 μl) were
incubated at 37 C in the presence of DNase Ӏ (0.002 U/μg of DNA). At predetermined time
points, a 10 μl aliquot of the sample solution was transferred to plastic tubes and mixed with 20
μl of 0.5 M EDTA solution to stop the degradation and then stored at -20 C until use. These
samples were run on a 6 % PAGE and stained with ethidium bromide. The density of DNA
bands was quantitatively evaluated using the Multi Gauge software (FUJIFILM, Tokyo, Japan).
DNA hydrogel (220 μg/10 μl) was prepared in plastic tubes and incubated at 37 C after addition
of solution containing DNase Ӏ (0.002 U/μg of DNA). At predetermined time points, supernatant
was removed, and amount of remaining DNA was evaluated by measuring absorbance of 260 nm
at 95 C.
Antigen presentation assay. To cultured DC2.4 cells were added DNA (2 g/ml) and OVA (2
mg/ml), then CD8OVA1.3 cells, then the mixture was incubated at 37 C in 5% CO2 for an
additional 24 h. The concentration of IL-2 in the supernatant was determined using an ELISA kit
(mouse IL-2 BD OptEIA Set, BD Biosciences).
Immunization of mice. Under anesthesia with isoflurane, the dorsal skin of C57BL/6 mice was
injected with 50 g OVA in the presence or absence of 220 g DNA in 10 l saline or with
complete Freund’s adjuvant (CFA). Mice were immunized thrice on days 0, 7, and 14. Seven
days after the last immunization, mice were killed and serum and the spleen were collected.
5
Measurement of OVA-specific antibody. Serum samples were serially diluted to measure the
OVA-specific total IgG levels by ELISA as previously described [23].
IFN- secretion from spleen cells. Seven days after the last immunization, spleen cells were
isolated, purified and cultured in the presence of OVA (1 mg/ml) in 96-well culture plates for 4
days. The concentration of IFN- in supernatant was determined by ELISA (Ready-SET-Go!
Mouse IFN- ELISA, eBioscience, San Diego, CA, USA).
Cytotoxic T lymphocyte assay. Seven days after the last immunization, spleen cells were
isolated and purified as above. To prime CTLs, splenocytes were co-cultured with mitomycin C-
treated EG7-OVA cells for 5 days in 5% CO2 at 37 C. Target cells (EG7-OVA or EL4) were
labeled with 51
Cr-sodium chromate (Na251
CrO4, Fujifilm RI Pharma, Tokyo, Japan). Boosted
splenocytes, effector cells, were serially diluted and co-incubated with the target cells for 4 h at
37 C. Then, the percentage of specific lysis was calculated as previously reported [20].
Hematoxylin and eosin staining of skin sections. Under anesthesia with isoflurane, the dorsal
skin of C57BL/6 mice was injected with 50 g OVA with or without 220 g DNA, CFA or 100
g alum (aluminum potassium sulfate dodecahydrate, Nacalai Tesque, Kyoto, Japan). Seven
days after the immunization, the injection site was excised, fixed in 4% paraformaldehyde,
embedded in paraffin, sliced and stained with hematoxylin and eosin. Stained samples were
examined under a microscope for histological evaluation.
Measurement of spleen weight. Spleen was collected from different sets of C57BL/6 mice at
seven days after the third immunization with weekly intervals. Spleen weight was measured as
an indicator of splenomegaly, a systemic adverse effect of immunostimulatory compounds.
Statistical analysis. Statistical analyses were performed using Statview v. 5.0 (SAS Institute Inc.,
Cary, NC, USA). Statistical differences were analyzed using one-way analysis of variance
(ANOVA) followed by Student-Newman-Keuls test. P values of 0.05 were considered
significant.
RESULTS
Spontaneous formation of DNA hydrogel. Several sets of ODNs were designed to obtain
polypodna preparations with three- (tripodna), four- (tetrapodna), or six-pods (hexapodna) (Table
S1). The formation of these preparations was confirmed by polyacrylamide gel electrophoresis
(PAGE) (Figure S1). Two sets of four ODNs with 40-nucleotide (nt) length in total and 12-nt
length of single stranded 5’-ends were used to obtain tetrapodna(CpG)12p-28-A and
tetrapodna(CpG)12np-28-A, respectively, and these were visualized using propidium iodide (PI), an
intercalating dye. A tetrapodna(CpG)12p-28-A having palindromic (p) 12-mer 5’-ends (5’-
acgtcatgacgt-3’) was soluble in a buffer solution containing 5 mM sodium chloride (Figure 1a,
far left), and gelled upon drop wise addition into a solution containing physiological salt
concentration (phosphate-buffered saline; 137 mM NaCl, 2.7 mM KCl, 10 mM Na2HPO4 and
1.76 mM KH2PO4, pH, 7.4) (Figure 1a, third from left). Another tetrapodna,
tetrapodna(CpG)12np-28-A, with non-palindromic (np) 12-mer 5’-ends (5’-acgtcagcgtta-3’)
diffused when added into the solution (Figure 1a, far right). A typical field emission scanning
6
electron microscopy image of the DNA hydrogel consisting of tetrapodna(CpG)12p-28-A clearly
shows that the DNA hydrogel has an ordered structure with abundant space within the gel
(Figure 1b).
Hydrogel formation by mixing two polypodna preparations. The mixing of a polypodna and
other DNA components with the 5’-ends complementary to the sequence of the polypodna will
lead to hydrogel formation. This mixing strategy is useful when considering the incorporation of
compounds into DNA hydrogels. Three types of hexapodna preparations, hexapodna(GpC)8np-32-
A, hexapodna(GpC)8np-32-B and hexapodna(GpC)8np-32-C, were designed; the first two shared
complementary 5’-ends (5’-tcctgacg-3’ and 5’-cgtcagga-3’), whereas the 5’-ends of the third
hexapodna were not complementary to either of the
other oligonucleotides. Figure 1c shows two sets of
PI-labeled hexapodna preparations mixed in a 29-
gauge syringe. When hexapodna(GpC)8np-32-A and
hexapodna(GpC)8np-32-B were mixed together,
DNA hydrogel (DNA hydrogel(GpC)) was quickly
formed (Figure 1c, right). The water content
calculated from the composition of the gel was
97.8 w/v%, indicating most of the component in
the gel is water. The Tm of the 8-mer 5’-ends of
hexapodna(GpC)8np-32-A and hexapodna(GpC)8np-
32-B was calculated to be 35.0C at DNA
concentration of 24.6 g/ml, whereas the Tm of
DNA hydrogel(GpC) was 55.8C at the same
concentration, suggesting that the hybridization of
the 8-mer 5’-ends of hexapodna preparations
consisting of DNA hydrogel is more thermally
stable than the hybridization of simple 8-mer
ODNs, even though the sequences are the same.
The injected DNA through the 29-gauge needle
almost instantly gelled (Figure 1d, right). As shown
in Figure 1e, DNA hydrogels were formed in the
skin tissues of mice. In contrast, the mixture of
non-complementary sets of hexapodna preparations
did not form hydrogels (Figure 1c left, Figure 1d
left, and Figure 1f). Similar results were obtained
using other polypodna preparations (data not
shown).
Figure 1. Formation of DNA hydrogel without DNA
ligase. (a) Hydrogel formation after drop wise addition of
tetrapodna preparations into a buffer solution. Tetrapodna
preparations were labeled using PI. Far left,
tetrapodna(CpG)12p-28-A in a buffer solution containing 5
mM sodium chloride. Second from the left, a solution
containing the physiological sodium chloride
concentration of 154 mM. Third from the left,
c
e
d
f
a
b
7
tetrapodna(CpG)12p-28-A added to the solution containing physiological sodium chloride concentration. Far
right, tetrapodna(CpG)12np-28-A added to the solution containing physiological sodium chloride concentration.
(b) An FE-SEM image of the inner structure of DNA hydrogel consisting of tetrapodna(CpG)12p-28-A. (c, d)
Hydrogel formation in syringe and injection through a 29-gauge needle. Hexapodna(GpC)8np-32-A and
hexapodna(GpC)8np-32-B (right, DNA hydrogel[GpC]) or hexapodna(GpC)8np-32-A and hexapodna(GpC)8np-32-C
(left), all of which were labeled using PI, were mixed in a 29-gauge insulin syringe (c), then injected (d). (e, f)
Hydrogel formation in mouse skin after intradermal injection. Hexapodna(GpC)8np-32-A and
hexapodna(GpC)8np-32-B (e, DNA hydrogel(GpC)) or hexapodna(GpC)8np-32-A and hexapodna(GpC)8np-32-C (f)
was injected into the dorsal skin of mice at a dose of 30 mg/kg (660 g/mouse), and the skin was collected and
observed at 3 h after injection.
Rapid recovery of the elasticity of DNA hydrogel on flow cessation. We next examined the
rheological behavior of the DNA hydrogel(GpC). For each experimental run, the hydrogel was
freshly prepared in a 29-gauge syringe at a total DNA concentration of 22.1 mg/ml (0.3 mM each
ODN/ml) and charged in the rheometer.
Figures 2a and 2b, respectively, show the storage and loss moduli (G’ and G’’) of the
hydrogel under oscillatory strain of various amplitudes (0) as indicated. In Figure 2b, the dotted
curves indicate the G’ data for 0 = 0.005 (0.5 %) and 0.1 (10%). For 0 ≤ 0.01 (1%), G’ is
independent of 0 and the angular frequency . Correspondingly, the loss modulus G” is much
smaller than G’, as noted from comparison of the triangles and upper dotted curve in Figure 2b.
This linear elastic behavior, characterized by the equilibrium modulus Ge = 1.1 103 Pa,
indicates the solid-like feature of the hydrogel due to the physical network of hexapodna units
not disputed under small strains.
In contrast, G’ begins to decrease whereas G’’ begins to increase with increasing 0 to 0.02
(2%). In particular, G’’ becomes well above G’ at the maximum strain amplitude examined, 0 =
0.1 (10 %), as noted from comparison of the filled squares and lower dotted curve in Figure 2b.
These features reflect nonlinear flow of the hydrogel under large strains. In relation to this
nonlinear flow, we also note that G’ for 0 = 0.1 exhibits a minimum at = 4 rad/s. This
minimum, rarely observed for ordinary physiological gels [24], suggests that the DNA hydrogel
has a molecular process with a characteristic time (in s) = 1/ = 0.25. The elasticity of the
hydrogel is undoubtedly sustained by the physical network of hexapodna units, and the large
strain should result in reorganization (disruption followed by reformation) of the network. This
reorganization appears to occur at = 0.25 s: For below 1/, the network has a sufficient time
to reform itself during one cycle of oscillation to exhibit larger G’. In contrast, for above 1/, it
has an insufficient time for disruption thereby exhibiting larger G’. The minimum of G’ at =
1/ possibly resulted from competition of such reformation and disruption processes.
Consequently, Figure 2b shows the G’’/G’ ratio for 0 = 0.1 to become the largest at = 1/,
which suggests that an efficiency thermal dissipation of the mechanical energy reflected in this
ratio becomes the highest when the network is most heavily disrupted.
The corresponding nonlinearity was noted also under constant-rate shear flow. Figure 2c
shows the stress +(t) of the hydrogel at a time t after start-up of the flow. The
+(t) data
measured for various rates are plotted against the strain imposed through the flow, = t. The
dashed line denotes the linear elastic response, + = Ge with Ge (= 1.1 10
3 Pa) being the
equilibrium modulus explained earlier. The +(t) data for all values follow this line for small
< 0.03. Thus the hydrogel behaves as an elastic solid even under flow, given that the strain does
8
not exceed a threshold, * 0.03. Interestingly,
this * value is close to the onset of nonlinearity
(0 0.02) under the oscillatory strain (Figure
2a). For > * in Figure 2c,
+ deviates
downward from the linear elastic line and decays
to a steady state value ss. This behavior reflects
the “yielding” (switch from solid to fluid) under
flow. In Figure 2d, those ss values are plotted
against the shear rate, . The ss data approach a
constant value of 13 Pa with decreasing , which
indicates that the hydrogel has a dynamic yield
stress, y,dyn 13 Pa, being necessary for
reorganizing the hydrogel under steady flow. The
y,dyn value is smaller than the static yield stress
required for the network reorganization under
slow strain, y,dyn 32 Pa (estimated in Figure 2c
as the stress at = * 0.03). Thus, the network
appears to be scarcer under flow than at
equilibrium. Nevertheless, oscillatory tests
following the steady flow showed that the
equilibrium network was recovered immediately
after cessation of the flow. This rapid
reformation and small value of y,dyn enable easy
injection of the DNA hydrogel into the mouse
through the syringe and solidification
immediately after the injection.
Figure 2. Rheological characterization of DNA
hydrogel exhibiting quick reorganization of
hydrogen bonds at room temperature (~25 C). (a)
and (b) Storage and loss moduli (G’ and G’’) measured
for sinusoidal strain at various angular frequencies
and with the amplitude 0 as indicated. In panels (a) and
(b), respectively, the G’ and G’’ data are plotted against
in the double-logarithmic scale. The dotted curves in
panel (b) indicate the G’ data for amplitude 0 = 0.005
and 0.1 (0.5% and 10 %). The minimum of G’ at = 4
s-1
observed for large 0 is indicative of the network
reorganization process at a characteristic time 0.25 s.
(c) Time evolution of the shear stress +(t) measured
after start-up of shear flow at constant rates as
indicated. The +(t) are plotted against the strain, = t. (d) Steady state shear stress ss evaluated from the
+(t) data shown in Fig. 2c. The ss data are plotted against the shear rate and the dynamic yield stress, y,dyn
13 Pa, is evaluated from those data at low . Data shown are representative of two independent experiments.
d
-2 -1 0 1
log
(ss/P
a)
0.5
1
1.5
2
log(/s-1)
c
log
-3 -2 -1 0 1 2
log
(
+(t
)/P
a)
0
1
2
3
0.1
0.2
0.4
0.8
1.6
3.2
/s-1
a
log (/rad s-1)
0 1 2
log
(G
’/P
a)
1
2
3
4
0.005
0.01
0.02
0.05
0.1
0
b
log (/rad s-1)
0 1 2
log
(G
’’/P
a)
1
2
3
4
0.005
0.01
0.02
0.05
0.1
0G' (0 = 0.005)
G' (0 = 0.1)
9
Increased immunostimulatory activity of CpG DNA by hydrogel formation. We previously
demonstrated that the immunostimulatory activity of CpG DNA is significantly increased by
conversion into polypodna [14,15,17,25]. To examine the immunostimulatory activity of DNA
hydrogels, several forms of DNA samples were compared in terms of interleukin-6 (IL-6) release
from mouse dendritic DC2.4 cells. Figure 3a shows the amount of IL-6 released from DC2.4
cells after addition of DNA samples at the indicated concentrations. Similar to the hexapodna
preparations with no single stranded 5’-ends15, hexapodna(CpG) induced a greater amount of
IL-6 production than ssDNA(CpG). At equimolar concentrations, DNA hydrogel(CpG) was
significantly (P < 0.05) more potent than hexapodna(CpG) in inducing IL-6. GpC samples
induced no detectable IL-6 production, irrespective of the structures.
Figure 3. IL-6 production, sustained delivery to regional lymph nodes, and upregulation of IL-6 mRNA
expression by DNA hydrogel(CpG). (a) IL-6 release from DC2.4 cells. Cells were incubated with DNA
samples at the indicated concentrations for 16 h. The IL-6 concentration in culture media was measured by
ELISA, and was 1.7 ± 0.9 pg/ml in untreated DC2.4 cells. Results are expressed as the mean ± S.D. of three
independent wells per sample. Data shown are representative of three independent experiments. All the data
obtained with DNA hydrogel(CpG) were statistically significant compared with the other groups. (b, c) Time
course of radioactivity in the injection site (b) and in draining lymph nodes (c) after intradermal injection of 32
P-DNA. Mice were injected with 32
P-ssDNA(CpG), 32
P-hexapodna(CpG) or 32
P-DNA hydrogel(CpG) at a
DNA dose of 10 mg/kg (220 μg/mouse) into the dorsal skin. At the indicated times, the skin tissue including
the injection site (b) and the draining lymph nodes (c) were collected, and radioactivity was counted. Data are
normalized to the injected dose and are expressed as the mean ± S.D. of three mice. Data shown are
representative of three independent experiments. (d, e) mRNA expression of IL-6 in the injection site (d) and
in draining lymph nodes (e) after intradermal injection of DNA. Mice were injected with DNA samples at a
dose of 220 μg/mouse into the dorsal skin. At the indicated times, the IL-6 mRNA expression was evaluated
by real-time PCR. Results are normalized to the internal control β-actin gene, and are expressed as the mean ±
S.D. of three or four mice. Data shown are representative of three independent experiments. *P < 0.05
compared with ssDNA(CpG) and all the GpC groups, #P < 0.05 compared with all the others at the same time
point.
10
Tissue distribution of DNA hydrogel in mice. To trace the tissue distribution of DNA samples
after injection into the dorsal skin of mice, ssDNA(CpG)8np-32-A1 was end-labeled with 32
P using
[-32
P]ATP and T4 polynucleotide kinase, and 32
P-labeled ssDNA(CpG), hexapodna(CpG), and
DNA hydrogel(CpG) were prepared as described above. Figure 3b shows the time course of 32
P
radioactivity in the dorsal skin of mice. After injection of 32
P-ssDNA(CpG) or 32
P-
hexapodna(CpG), 32
P radioactivity quickly
disappeared from the injection site. In stark contrast, 32
P radioactivity remained at the injection site for a
longer period after injection of 32
P-DNA
hydrogel(CpG) with a half-life of about 12 h. The
injection of 32
P-DNA hydrogel(CpG) resulted in a
slow and sustained accumulation of 32
P radioactivity
in the lymph nodes (Figure 3c).
Correlation between tissue distribution of CpG
DNA and elevated IL-6 expression. An injection of
ssDNA(CpG) resulted in a slight increase in the
mRNA expression (Figure 3d). On the other hand, an
injection of hexapodna(CpG) or DNA hydrogel(CpG)
significantly increased the IL-6 expression at the
injection site 6 h after injection. The expression
remained high for the experimental period of 24 h
only in the DNA hydrogel(CpG) group. Similar
profiles of IL-6 mRNA expression were observed in
the draining lymph nodes (Figure 3e). There was no
large increase in the IL-6 concentration in the serum
after injection of DNA samples into the dorsal skin
(Figure S2), indicating that DNA hydrogel(CpG)
induces IL-6 expression at local sites where they
accumulate.
Figure 4. OVA release from DNA hydrogel and antigen
presentation in dendritic cells. (a, b) Time course of OVA
release from DNA hydrogel. FITC-OVA (50 g) was
encapsulated into 220 g of DNA hydrogel(CpG) and placed
into the upper chamber of the Transwell (0.4 m pore size)
with the bottom chamber containing PBS, and incubated at 37
C. The bright field (a, upper) and fluorescent images (a,
lower) of the gel were photographed at the indicated times.
The concentration of FITC-OVA in the bottom chamber was
measured and plotted against time (b). Results are expressed
as the mean ± S.D. of three wells per sample. Data shown are
representative of three independent experiments. (c)
Degradation of DNA hydrogel and hexapodna by DNase I.
DNA samples were incubated at 37 C in the presence of
DNase I and the remaining amounts of DNA were plotted
0 h 1 h 6 h 12 h 24 h
a
d
b
c
IL-2
(pg/m
l)
0
5
10
15
20
25*
Time (h)
0 6 12 18 24
OV
A rele
ase
(%
)
0
50
100
Time (h)
0 6 12 18 24
Rem
ain
ing D
NA
(%
)
0
50
100
Hydrogel
(–DNase)
Hydrogel
Hexapodna
11
against time. Results are expressed as mean S.D. of three independent determinations per sample. (d) IL-2
secretion from CD8OVA1.3 cells. DC2.4 cells (5 104 cells/well) were added with OVA (2 mg/ml) and CpG
DNA (2 g/ml), and incubated for 24 h. Thereafter, CD8OVA1.3 cells (5 104 cells/well) were added to each
well and incubated for an additional 24 h. The IL-2 concentration in culture media was measured by ELISA.
Results are expressed as the mean ± S.D. of three independent determinations per sample. Data shown are
representative of two independent experiments. *P < 0.05 compared with the OVA alone group.
Sustained release of OVA from DNA hydrogel. In order to visualize OVA release, we first
encapsulated fluorescein isothiocyanate (FITC)-labeled OVA, a model antigen, into DNA
hydrogel(CpG) consisting of hexapodna(CpG)8np-32-A and hexapodna(CpG)8np-32-B. Figure 4a
shows the bright-field and fluorescent images of FITC-OVA/DNA hydrogel(CpG). The hydrogel
was swollen for the first 1 h, and a yellow color representing FITC-OVA was gradually diluted
with time. The fluorescent images clearly show the slow release of FITC-OVA from DNA
hydrogel(CpG). The fluorescence intensity measurement showed that FITC-OVA was gradually
released from the DNA hydrogel (Figure 4b) with a half-life of 2.5 h (Figure S3). Figure 4c
shows the degradation of DNA hydrogel(CpG) and hexapodna(CpG)8np-32-A in buffer solution
with or without DNase I. DNA hydrogel(CpG) was much more resistant to degradation than
hexapodna(CpG)8np-32-A.
Enhanced presentation of OVA by DNA hydrogel. DC2.4 mouse dendritic cells were
incubated with OVA in the presence or absence of DNA, and then CD8OVA1.3 T hybridoma
cells that recognize an OVA peptide (OVA257–264) were added and incubated for additional 24 h.
The addition of ssDNA(CpG), hexapodna(CpG) or DNA hydrogel(CpG) resulted in a significant
increase in IL-2 production compared with the OVA group (Figure 4d).
Induction of anti-OVA immune response in mice. Mice were immunized with OVA with or
without DNA by three intradermal injections at weekly intervals. Complete Freund’s adjuvant
(CFA), which is highly potent but severely toxic, was used as a positive control. DNA
hydrogel(CpG) significantly increased the OVA specific total IgG titer in mouse serum
compared with ssDNA(CpG) or hexapodna(CpG) groups (Figure 5a). Splenocytes of mice
immunized with OVA/DNA hydrogel(CpG) produced significantly higher amounts of IFN-
compared with those immunized with other formulations after restimulation with OVA (Figure
5b). The immunization with OVA/DNA hydrogel(CpG) induced significant cytotoxic T
lymphocyte (CTL) responses against EG7-OVA cells, a cell line derived from the murine
lymphoma EL-4 cells transfected with OVA cDNA (Figure 5c) but not against EL4 cells (Figure
5d). When OVA and DNA hydrogel(CpG) were administered separately to the dorsal skin
(OVA) and to the footpad (DNA hydrogel), all the parameters examined were lower than those
of the combined OVA/DNA hydrogel(CpG) group (Figure S4). OVA/DNA hydrogel(CpG)
induced no significant changes at the injection site or in spleen weight, in contrast to OVA
injected with CFA or alum, which is used in some vaccine formulations (Figure S5).
12
Figure 5. Induction of OVA specific immune responses after intradermal injection of OVA into mice. (a)
OVA-specific total IgG in mouse serum after immunization. Mice were immunized with OVA with or without
DNA by three intradermal injections at weekly intervals. At 7 days after the last immunization, the OVA-
specific total IgG levels in serum were measured by ELISA. Serum total IgG titers were estimated by the
dilution ratio at which the absorbance value of the saline group was obtained. Results are expressed as mean ±
S.D. of three or four mice. Data shown are representative of three independent experiments. #P < 0.05
compared with all the other OVA/DNA groups. (b) IFN- production from splenocytes after re-stimulation
with OVA. At seven days after the last immunization, splenocytes collected were added with OVA (1 mg/ml),
and incubated for 4 days. The IFN- concentration in culture media was measured by ELISA. Results are
expressed as mean ± S.D. of three or four mice. Data shown are representative of two independent experiments.
#P < 0.05, statistically significant compared with the other groups. (c, d) CTL activity after immunization of
mice with OVA. Seven days after the last immunization, splenocytes collected (5 107 cells) were co-cultured
with mitomycin C-treated EG7-OVA (5 106 cells) for 5 days. EG7-OVA (c) or EL4 (d) were labeled with
51Cr as target cells and co-incubated with the effector cells at the indicated ratio for 4 h. Results are expressed
as mean ± S.D. of three or four mice. Data shown are representative of two independent experiments. *P <
0.05 compared with the OVA alone group.
DISCUSSION
Recent development of DNA nanotechnology has produced a large variety of DNA-based nano-
and macrosystems [26-29]. One such system is DNA hydrogel, and several groups, including
ours, have reported preparative methods and applications of DNA hydrogel systems [16-19]. The
DNA-based material developed here was the hydrogel exhibiting the elasticity under small strain
as shown in Figure 2a. In addition, the material did not flow with its own weight but was easily
injected through a fine-gauged needle, which also indicates that the material is a gel. The DNA
hydrogel developed in the present study has several unique and superior properties to other DNA
hydrogels. First, it is injectable through an extra-fine, 29-gauge syringe. Injectable systems are
much better than implantable ones when administered to patients. Second, no chemicals or
synthetic compounds are needed for hydrogel preparation and gelation. Short DNA are the only
components of the hydrogel, except for water and salts; this greatly enhances biocompatibility
and biodegradability. Finally, hydrogel is an important system for sustained delivery of bioactive
compounds [30-32]. Thus, the DNA hydrogel developed in this study provides a useful system
for their sustained delivery. Some superior properties of the DNA hydrogel are attributed to the
structural and thermal properties of nano-sized polypodna preparations that are designed and
constructed using DNA nanotechnology. As demonstrated herein, DNA hydrogel can be
developed either as an immunostimulatory system or in an immunologically inert mode.
The lower activity of hexapodna indicates that (1) DNA hydrogel is actually formed after
injection, and (2) gel formation is important for the induction of OVA-specific immune
13
responses. Clearance of topically injected DNA is mediated mainly by DNase-mediated
degradation and by absorption into systemic circulation [33]. Gel formation interferes with the
degradation because of the reduced free terminals as well as of steric hindrance. The absorption
of compounds from the injection site is a function of molecular size, so that gel formation is a
requisite for the slow clearance of DNA samples. At that point, OVA or other incorporated
molecules can then be slowly released from the hydrogel. Since Liu et al. demonstrated that
assembled antigen-CpG DNA complexes were useful for inducing antigen-specific antibody
responses [34], conjugates or complexes of OVA and CpG hexapodna may also be useful for the
induction of OVA-specific immune responses. This possibility will be examined in future studies.
Crucially, we found that the DNA hydrogel undergoes very quick network reformation.
Analysis of the modulus data suggested that the hydrogel is reorganized in a time scale of 0.25 s.
This property is quite different from that of most hydrogel systems [24]. When the hydrogel is
stressed, a fraction of the bonds is dissociated and, at the same time, the resulting free ends
change partner and quickly reassociate through hydrogen bonds. This dissociation/association
process allows the DNA hydrogel to be injected through an extra-fine needle and to return
quickly to the gel state after injection.
The sharp difference between DNA hydrogel(CpG) and DNA hydrogel(GpC) clearly
indicate that the recognition of CpG DNA by TLR9 is involved in the OVA-specific immune
responses. Several studies using CpG DNA (which in most cases is phosphorothioate-modified)
showed that the immunostimulation is important for antigen-specific immune responses [35-37].
The limited functions of ssDNA or hexapodna indicate that sustained OVA release is critical for
induction of OVA-specific immune responses.
DNA hydrogel can be prepared from a wide variety of ODNs that can be custom-designed
to fit the specific purpose. Thus, although our hydrogel described here was very effective, we
cannot yet conclude that it is optimized for the induction of OVA-specific immune responses.
This is since all the properties of DNA hydrogel, i.e., the immunostimulatory activity, the release
rate of OVA, in vivo stability/degradation, are determined by its components. The optimization
of these properties should be examined in future studies.
CONCLUSIONS
We have developed an injectable, self-gelling, biodegradable, and immunostimulatory DNA
hydrogel using ODNs containing immunostimulatory CpG motifs, and proved that the hydrogel
is an efficient system for sustained delivery of OVA, and for induction of the antigen-specific
immune responses. Because the gel formation can be controlled by the salt concentration, the
hydrogel can be delivered not only via injection but also packaged in spray or inhalation
applications.
ACKNOWLEDGMENTS
This work was supported in part by a Grant-in-Aid for Scientific Research (B) (23390010) from
Japan Society for the Promotion of Science (JSPS) and by a Grant-in-Aid for Scientific Research
on Innovative Areas “Carcinogenic spiral” (25114706) from Ministry of Education, Culture,
Sports, Science and Technology of Japan.
14
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17
FIGURE LEGENDS
Figure 1. Formation of DNA hydrogel without DNA ligase. (a) Hydrogel formation after drop
wise addition of tetrapodna preparations into a buffer solution. Tetrapodna preparations were
labeled using PI. Far left, tetrapodna(CpG)12p-28-A in a buffer solution containing 5 mM sodium
chloride. Second from the left, a solution containing the physiological sodium chloride
concentration of 154 mM. Third from the left, tetrapodna(CpG)12p-28-A added to the solution
containing physiological sodium chloride concentration. Far right, tetrapodna(CpG)12np-28-A
added to the solution containing physiological sodium chloride concentration. (b) An FE-SEM
image of the inner structure of DNA hydrogel consisting of tetrapodna(CpG)12p-28-A. (c, d)
Hydrogel formation in syringe and injection through a 29-gauge needle. Hexapodna(GpC)8np-32-
A and hexapodna(GpC)8np-32-B (right, DNA hydrogel[GpC]) or hexapodna(GpC)8np-32-A and
hexapodna(GpC)8np-32-C (left), all of which were labeled using PI, were mixed in a 29-gauge
insulin syringe (c), then injected (d). (e, f) Hydrogel formation in mouse skin after intradermal
injection. Hexapodna(GpC)8np-32-A and hexapodna(GpC)8np-32-B (e, DNA hydrogel(GpC)) or
hexapodna(GpC)8np-32-A and hexapodna(GpC)8np-32-C (f) was injected into the dorsal skin of
mice at a dose of 30 mg/kg (660 g/mouse), and the skin was collected and observed at 3 h after
injection.
Figure 2. Rheological characterization of DNA hydrogel exhibiting quick reorganization of
hydrogen bonds at room temperature (~25 C). (a) and (b) Storage and loss moduli (G’ and
G’’) measured for sinusoidal strain at various angular frequencies and with the amplitude 0 as
indicated. In panels (a) and (b), respectively, the G’ and G’’ data are plotted against in the
double-logarithmic scale. The dotted curves in panel (b) indicate the G’ data for amplitude 0 =
0.005 and 0.1 (0.5 % and 10 %). The minimum of G’ at = 4 s-1
observed for large 0 is
indicative of the network reorganization process at a characteristic time 0.25 s. (c) Time
evolution of the shear stress +(t) measured after start-up of shear flow at constant rates as
indicated. The +(t) are plotted against the strain, = t. (d) Steady state shear stress ss
evaluated from the +(t) data shown in Fig. 2c. The ss data are plotted against the shear rate
and the dynamic yield stress, y,dyn 13 Pa, is evaluated from those data at low . Data shown
are representative of two independent experiments.
Figure 3. IL-6 production, sustained delivery to regional lymph nodes, and upregulation of
IL-6 mRNA expression by DNA hydrogel(CpG). (a) IL-6 release from DC2.4 cells. Cells were
incubated with DNA samples at the indicated concentrations for 16 h. The IL-6 concentration in
culture media was measured by ELISA, and was 1.7 ± 0.9 pg/ml in untreated DC2.4 cells.
Results are expressed as the mean ± S.D. of three independent wells per sample. Data shown are
representative of three independent experiments. All the data obtained with DNA hydrogel(CpG)
were statistically significant compared with the other groups. (b, c) Time course of radioactivity
in the injection site (b) and in draining lymph nodes (c) after intradermal injection of 32
P-DNA.
Mice were injected with 32
P-ssDNA(CpG), 32
P-hexapodna(CpG) or 32
P-DNA hydrogel(CpG) at
a DNA dose of 10 mg/kg (220 μg/mouse) into the dorsal skin. At the indicated times, the skin
tissue including the injection site (b) and the draining lymph nodes (c) were collected, and
radioactivity was counted. Data are normalized to the injected dose and are expressed as the
mean ± S.D. of three mice. Data shown are representative of three independent experiments. (d,
e) mRNA expression of IL-6 in the injection site (d) and in draining lymph nodes (e) after
intradermal injection of DNA. Mice were injected with DNA samples at a dose of 220 μg/mouse
18
into the dorsal skin. At the indicated times, the IL-6 mRNA expression was evaluated by real-
time PCR. Results are normalized to the internal control β-actin gene, and are expressed as the
mean ± S.D. of three or four mice. Data shown are representative of three independent
experiments. *P < 0.05 compared with ssDNA(CpG) and all the GpC groups, #P < 0.05
compared with all the others at the same time point.
Figure 4. OVA release from DNA hydrogel and antigen presentation in dendritic cells. (a,
b) Time course of OVA release from DNA hydrogel. FITC-OVA (50 g) was encapsulated into
220 g of DNA hydrogel(CpG) and placed into the upper chamber of the Transwell (0.4 m
pore size) with the bottom chamber containing PBS, and incubated at 37 C. The bright field (a,
upper) and fluorescent images (a, lower) of the gel were photographed at the indicated times.
The concentration of FITC-OVA in the bottom chamber was measured and plotted against time
(b). Results are expressed as the mean ± S.D. of three wells per sample. Data shown are
representative of three independent experiments. (c) Degradation of DNA hydrogel and hexapodna by
DNase I. DNA samples were incubated at 37 C in the presence of DNase I and the remaining amounts of
DNA were plotted against time. Results are expressed as mean S.D. of three independent determinations per
sample. (d) IL-2 secretion from CD8OVA1.3 cells. DC2.4 cells (5 104 cells/well) were added
with OVA (2 mg/ml) and CpG DNA (2 g/ml), and incubated for 24 h. Thereafter, CD8OVA1.3
cells (5 104 cells/well) were added to each well and incubated for an additional 24 h. The IL-2
concentration in culture media was measured by ELISA. Results are expressed as the mean ±
S.D. of three independent determinations per sample. Data shown are representative of two
independent experiments. *P < 0.05 compared with the OVA alone group.
Figure 5. Induction of OVA specific immune responses after intradermal injection of OVA
into mice. (a) OVA-specific total IgG in mouse serum after immunization. Mice were
immunized with OVA with or without DNA by three intradermal injections at weekly intervals.
At 7 days after the last immunization, the OVA-specific total IgG levels in serum were measured
by ELISA. Serum total IgG titers were estimated by the dilution ratio at which the absorbance
value of the saline group was obtained. Results are expressed as mean ± S.D. of three or four
mice. Data shown are representative of three independent experiments. #P < 0.05 compared with
all the other OVA/DNA groups. (b) IFN- production from splenocytes after re-stimulation with
OVA. At seven days after the last immunization, splenocytes collected were added with OVA (1
mg/ml), and incubated for 4 days. The IFN- concentration in culture media was measured by
ELISA. Results are expressed as mean ± S.D. of three or four mice. Data shown are
representative of two independent experiments. #P < 0.05, statistically significant compared with
the other groups. (c, d) CTL activity after immunization of mice with OVA. Seven days after the
last immunization, splenocytes collected (5 107 cells) were co-cultured with mitomycin C-
treated EG7-OVA (5 106 cells) for 5 days. EG7-OVA (c) or EL4 (d) were labeled with
51Cr as
target cells and co-incubated with the effector cells at the indicated ratio for 4 h. Results are
expressed as mean ± S.D. of three or four mice. Data shown are representative of two
independent experiments. *P < 0.05 compared with the OVA alone group.